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Research sites –  SELF-ASSEMBLING NANOEMULSIONS -- data collected mostly at following institutions: 1)		Research School of Physical Sciences 		Australian National Univ.;  Canberra, Australia 2)		Dept. of Surgery,  Div. of Neurosurgery 		Univ. of Connecticut Health Ctr.;  Farmington, CT 3)		Dept. of Neurosurgery,  Hartford Hospital;  CT ( chronology same as “slide order” below ):
set-up for    Langmuir trough set-up for lipid monolayer analysis                      (  Stable  Nanoemulsions,   2010,   3rd  edition,   Elsevier,    --  [ Fig.  6.1 ]  )
ff1       Surface pressure-area curves for a microbubble-surfactant monolayer spread at air/water interface
fffffffffffffffffff1 Surface pressure-area curves for microbubble surfactant monolayers spread on aqueous phases
fffffffffffffffffff5
	   ARTIFICIAL  “MIXED-LIPID”  NANOEMULSIONS: Self-assembly  using  ONLY  NONionic  lipids; Contains  both  submicron-sized 		1)  lipid-coated  microbubbles, and 		2)  liquid-crystal  microparticles  predominantly 	( and both labeled “LCM” in slides below); Lipids employed consist of glycerides, cholesterol, and cholesterol esters  (but NOT phospholipids).
  Lipid-coated microbubble histograms (from flow cytometer): A) saturated solution of FilmixTM lipid mixture;   B) distilled water alone;   C) computed “difference histogram” of LCM.
   Relative size distribution of LCM:  Unstirred medium. (Light-scatter signals collected during 1,000-sec period.)
      Relative size distribution of LCM:  Stirred medium. (Light-scatter signals collected during 1,000-sec. period.)
`````````````````````````````````````````````  Direct  optical  imaging  of  lipid-coated  microbubbles  (LCM) 	  by  phase-measurement   interferometric   microscopy.
	   TARGETED  DRUG  DELIVERY  using  a  STABLE  LIPID  NANOEMULSION  vehicle: Lipid  nanoemulsion  targets  certain “lipoprotein  receptors”; Drug delivery to target cells is by “ACTIVE uptake” process  --  i.e., by ENDOCYTOSIS; LCM uptake by target cells is rapid  (-- often     2 minutes after i.v. injection in rats).
Microbubble count contour map.  Lipid-coated microbubble (LCM) distribution in tumor -- represented by lines of microbubbleisodensity in contour map (bottom right).
  Tumor targeting ability of LCM, after i.v. injection, in rat with liver tumor.  (Stained LCM appear here as solid black discs.)
   Confinement of LCM to 9L-gliosarcoma (top left) and to C6-glioma (top right) in rats.  Bottom panels show 9L tumor with diO-labeled LCM, in rat, by confocal laser microscopy.
Interactions of LCM with cultured tumor cells. C6 cells with diO-LCM (panelsA,B) or diO alone (panels C,D)
Kinetics of LCM uptake by tumor cells in culture. ( C6 glioma cells incubated with diO-LCM at 3 temper-atures for periods ranging from 5 to 60 minutes. )
	Localization of diO-LCM in intracellular acidic com-partments.  ( C6 tumor cell seen using  dual-mode recording for diO [A] and TR stains [B]. Bar = 10 µm)
nnnn     Effects of paclitaxel-loaded LCM on the C6-tumor cell morphology.   (Control culture [top panel];  paclitaxel [bottom left panel];   paclitaxel-LCM [bottom right].)
	Photomicrograph demonstrating tumor morphology of  Sprague-Dawley  rats  bearing  C6  glioma  treated with  paclitaxel-CRE  (A),  and  paclitaxel- LCM  (B, C).
Photomicrograph  demonstrating  tumor  morphology 	of Fischer 344 rats bearing 9L gliosarcomas treated 	with cremophor-LCM (A),  and paclitaxel-LCM (B,C).
Summary  of  findings  on  STABLE, MIXED-LIPID, “LCM/nanoparticle-derived” NANOEMULSIONS: ,[object Object]
Display marked capability for rapid (actively) 	targeted chemotherapy;
Selective uptake by target cells occurs via 	“lipoprotein receptor”-mediated endocyto-	sis (particularly via scavenger receptors);
Long-lived (liquid-crystalline) lipid nanostruc-	tures predominate in the submicron range	[ cf.  particle-size-distribution  slides  below ].

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Stable nanoemulsions slide show (ppt)

  • 1. Research sites – SELF-ASSEMBLING NANOEMULSIONS -- data collected mostly at following institutions: 1) Research School of Physical Sciences Australian National Univ.; Canberra, Australia 2) Dept. of Surgery, Div. of Neurosurgery Univ. of Connecticut Health Ctr.; Farmington, CT 3) Dept. of Neurosurgery, Hartford Hospital; CT ( chronology same as “slide order” below ):
  • 2. set-up for Langmuir trough set-up for lipid monolayer analysis ( Stable Nanoemulsions, 2010, 3rd edition, Elsevier, -- [ Fig. 6.1 ] )
  • 3. ff1 Surface pressure-area curves for a microbubble-surfactant monolayer spread at air/water interface
  • 4. fffffffffffffffffff1 Surface pressure-area curves for microbubble surfactant monolayers spread on aqueous phases
  • 6.
  • 7. ARTIFICIAL “MIXED-LIPID” NANOEMULSIONS: Self-assembly using ONLY NONionic lipids; Contains both submicron-sized 1) lipid-coated microbubbles, and 2) liquid-crystal microparticles predominantly ( and both labeled “LCM” in slides below); Lipids employed consist of glycerides, cholesterol, and cholesterol esters (but NOT phospholipids).
  • 8. Lipid-coated microbubble histograms (from flow cytometer): A) saturated solution of FilmixTM lipid mixture; B) distilled water alone; C) computed “difference histogram” of LCM.
  • 9. Relative size distribution of LCM: Unstirred medium. (Light-scatter signals collected during 1,000-sec period.)
  • 10. Relative size distribution of LCM: Stirred medium. (Light-scatter signals collected during 1,000-sec. period.)
  • 11. ````````````````````````````````````````````` Direct optical imaging of lipid-coated microbubbles (LCM) by phase-measurement interferometric microscopy.
  • 12. TARGETED DRUG DELIVERY using a STABLE LIPID NANOEMULSION vehicle: Lipid nanoemulsion targets certain “lipoprotein receptors”; Drug delivery to target cells is by “ACTIVE uptake” process -- i.e., by ENDOCYTOSIS; LCM uptake by target cells is rapid (-- often 2 minutes after i.v. injection in rats).
  • 13. Microbubble count contour map. Lipid-coated microbubble (LCM) distribution in tumor -- represented by lines of microbubbleisodensity in contour map (bottom right).
  • 14. Tumor targeting ability of LCM, after i.v. injection, in rat with liver tumor. (Stained LCM appear here as solid black discs.)
  • 15. Confinement of LCM to 9L-gliosarcoma (top left) and to C6-glioma (top right) in rats. Bottom panels show 9L tumor with diO-labeled LCM, in rat, by confocal laser microscopy.
  • 16. Interactions of LCM with cultured tumor cells. C6 cells with diO-LCM (panelsA,B) or diO alone (panels C,D)
  • 17. Kinetics of LCM uptake by tumor cells in culture. ( C6 glioma cells incubated with diO-LCM at 3 temper-atures for periods ranging from 5 to 60 minutes. )
  • 18. Localization of diO-LCM in intracellular acidic com-partments. ( C6 tumor cell seen using dual-mode recording for diO [A] and TR stains [B]. Bar = 10 µm)
  • 19. nnnn Effects of paclitaxel-loaded LCM on the C6-tumor cell morphology. (Control culture [top panel]; paclitaxel [bottom left panel]; paclitaxel-LCM [bottom right].)
  • 20. Photomicrograph demonstrating tumor morphology of Sprague-Dawley rats bearing C6 glioma treated with paclitaxel-CRE (A), and paclitaxel- LCM (B, C).
  • 21. Photomicrograph demonstrating tumor morphology of Fischer 344 rats bearing 9L gliosarcomas treated with cremophor-LCM (A), and paclitaxel-LCM (B,C).
  • 22.
  • 23. Display marked capability for rapid (actively) targeted chemotherapy;
  • 24. Selective uptake by target cells occurs via “lipoprotein receptor”-mediated endocyto- sis (particularly via scavenger receptors);
  • 25. Long-lived (liquid-crystalline) lipid nanostruc- tures predominate in the submicron range [ cf. particle-size-distribution slides below ].